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首页> 外文期刊>Journal of International Medical Research >Genetically-engineered mesenchymal stem cells transfected with human HCN1 gene to create cardiac pacemaker cells
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Genetically-engineered mesenchymal stem cells transfected with human HCN1 gene to create cardiac pacemaker cells

机译:转染人类HCN1基因的基因工程间充质干细胞创建心脏起搏器细胞

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摘要

Objective To test the proof-of-principle that genetically-engineered mesenchymal stem cells (MSCs) transfected with the human hyperpolarization-activated cyclic nucleotide-gated channel 1 (hHCN1) gene can be modified to become cardiac pacemaker cells. Methods MSCs were transfected with the hHCN1 gene using lentiviral-based transfection. The expressed pacemaker current (I f) in hHCN1-transfected MSCs was recorded using whole-cell patch-clamp analysis. The effect of the hHCN1-transfected MSCs on cardiomyocyte excitability was determined by coculturing the MSCs with neonatal rabbit ventricular myocytes (NRVM). The spontaneous action potentials of the NRVM were recorded by whole-cell current-clamp analysis. Results A high level time- and voltage-dependent inward hyperpolarization current that was inhibited by 4?mM caesium chloride was detected in hHCN1-transfected MSCs, suggesting that the HCN1 proteins acted as I f channels in MSCs. The mean?±?SE beating frequency in NRVMs cocultured with control MSCs transfected with the pcDNA3 plasmid control was 82?±?8 beats/min (n?=?5) compared with 129?±?11 beats/min (n?=?5) in NRVMs cocultured with hHCN1-transfected MSCs. Conclusions Genetically-engineered MSCs transfected with the hHCN1 gene can be modified to become cardiac pacemaker cells.
机译:目的检验原理,证明可以将转染人超极化激活环核苷酸门控通道1(hHCN1)基因的基因工程间充质干细胞(MSC)修饰为心脏起搏器细胞。方法以慢病毒为基础的hHCN1基因转染MSC。使用全细胞膜片钳分析记录在hHCN1转染的MSC中表达的起搏器电流(I f)。 hHCN1转染的MSC对心肌细胞兴奋性的影响是通过将MSC与新生兔心室肌细胞(NRVM)共培养来确定的。通过全细胞电流钳分析来记录NRVM的自发动作电位。结果在hHCN1转染的MSC中检测到了高水平的时间和电压依赖性内向超极化电流,该电流被4μmM氯化铯抑制,这表明HCN1蛋白在MSC中充当了I f通道。与用pcDNA3质粒对照转染的对照MSC共培养的NRVM中的平均±±SE跳动频率为82±±8次/分(n == 5),而129±±11次/分(n ==)。 (5)与hHCN1转染的MSC共培养的NRVM中。结论转染了hHCN1基因的基因工程MSC可以被修饰成心脏起搏器细胞。

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